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Journal of Virology, September 2005, p. 11962-11973, Vol. 79, No. 18
0022-538X/05/$08.00+0     doi:10.1128/JVI.79.18.11962-11973.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.

An Authentic 3' Noncoding Region Is Necessary for Efficient Poliovirus Replication

David M. Brown, Christopher T. Cornell, Genevieve P. Tran, Joseph H. C. Nguyen, and Bert L. Semler^*

Department of Microbiology and Molecular Genetics, School of Medicine, University of California, Irvine, California 92697

Received 13 April 2005/ Accepted 29 June 2005

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

 
Picornavirus RNA replication involves the specific synthesis of negative-strand intermediates followed by an accumulation of positive-strand viral RNA in the presence of a multitude of cellular mRNAs. Previously, in an effort to identify cis-acting elements required for initiation of negative-strand RNA synthesis, we deleted the entire 3' noncoding regions from human rhinovirus and poliovirus genomic RNAs. These deletion mutation transcripts displayed a severe delay in RNA accumulation following transfection of HeLa cells. Interestingly, in subsequent infection of HeLa cells, the deletion-mutant poliovirus displayed only a moderate deficiency in RNA synthesis. These data suggested that the delay in the production of cytopathic effects after transfection may have been due to an RNA replication defect overcome by the accumulation of a compensatory mutation(s) generated during initial rounds of RNA synthesis. In this study, we have sequenced the entire genome of the deletion-mutant virus and found only two nucleotide changes from the parental clone. Transfection analysis of these sequence variants revealed that the sequence changes did not provide compensatory functions for the 3' noncoding region deletion mutation replication defect. Further examination of the deletion mutant phenotype revealed that the severe replication defect following RNA transfection is due, in part, to nonviral terminal sequences present in the in vitro-derived deletion mutation transcripts. Our data suggest that poliovirus RNA harboring a complete 3' noncoding region deletion mutation is infectious (not merely quasi-infectious).

	INTRODUCTION

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In the first step of poliovirus (PV) RNA replication, viral and host cell proteins form a membranous replication complex in which positive-strand viral RNA is used as the template to generate full-length, negative-strand RNA. The viral RNA polymerase (3D^pol) has been shown to be necessary and sufficient for elongation of an oligo(U)-primed, polyadenylated RNA template in vitro (17). Furthermore, the viral polymerase can nonspecifically generate the reverse complement of nonviral polyadenylated RNAs when provided with oligo(U) (13, 50). Because the replication complex discriminates between the biochemically similar 3' ends of cellular polyadenylated mRNAs and the polyadenylated PV genome, a cis-acting RNA replication element is thought to be required for template selection and the proper assembly of the replication initiation complex.

Within the family Picornaviridae, several RNA elements involved in genomic replication have been described. A stem-loop structure required for viral RNA replication was identified within the capsid-coding sequence of human rhinovirus 14 (35, 36). This replication element, termed cre, is located about 2.3 kb downstream from the 5' end and more than 4 kb from the 3' end of the genome. Elements with similar structures have been described in a number of other picornaviruses, each containing a conserved AAACA motif (21, 22, 33, 46). In PV1, the cre is located in the coding region of the nonstructural protein 2C. Additional studies have shown that the in vitro uridylylation of the viral protein VPg is greatly stimulated by the presence of the PV1 cre (46). The uridylylated form of VPg has long been thought to act as a protein primer for both positive-strand and negative-strand RNA synthesis, suggesting that the cre is necessary for the uridylylation of VPg during a PV infection.

Another replication element is found in enterovirus sequences corresponding to nucleotides 1 to 100 of the positive-strand genomic RNA (3, 74). This element is confined within stem-loop I of the PV 5' NCR (noncoding region) (24) and has a cloverleaf-like structure (3). This RNA structure binds viral protein 3CD and host protein PCBP, forming a ribonucleoprotein complex (2, 19, 45). Mutational analysis of the cloverleaf RNA suggests that the ribonucleoprotein complex is required for RNA replication (2, 54, 56) by acting either in cis for negative-strand synthesis (7, 20) or in trans for positive-strand synthesis (3). In addition, a ribonucleoprotein complex has also been shown to form at the 3' end of the complementary negative-strand RNA (9, 54). Further complicating the analysis, mutations of the cloverleaf structure have resulted in defects in cap-independent translation of the poliovirus genome (45, 60). It has also been suggested that the 5' cloverleaf ribonucleoprotein complex is involved in RNA stability (40), which would indirectly account for the apparent role in both replication and translation. Whether direct or indirect, the mechanism by which the PV 5' cloverleaf contributes to genomic replication has not been fully elucidated.

These findings highlight several important aspects of replication elements in picornaviruses. First, conserved sequences and structures involved in RNA replication need not be merely targeting signals that recruit the RNA genome to the replication complex but can be functional elements in any number of essential processes in the replication cycle. Second, functional RNA structure elements may be contained in the positive strand, the negative strand, or both strands of complementary RNAs. In addition, elements involved in RNA replication need not be close (in terms of linear sequence) to the sites of RNA replication initiation. Finally, picornavirus genomes contain multiple RNA replication element sequences, with each one likely to have a unique function.

For several reasons, the PV 3' NCR is a logical candidate to encode a cis-acting replication element that is required for the initiation of negative-strand RNA synthesis. Binding of the PV 3' NCR to components within the replication complex could be responsible for bringing the 3' poly(A) tract into close proximity to the 3D^pol to initiate negative-strand synthesis. Furthermore, while the PV 3' NCR is presumably not subject to the selective pressure of codon maintenance, there is a high degree of sequence conservation among the genomic 3' NCRs of the three PV serotypes. Such sequence conservation suggests that a strong selection pressure, like the preservation of a cis-acting replication element, is important in maintaining the primary structure (and therefore secondary structure and/or tertiary structure) of this region of the viral genome. Finally, it is likely that a conserved RNA motif is required for the replication complex to discriminate between PV genomic RNA and the multitude of cellular mRNAs. While there are at least two cis-acting replication elements in the PV1 genome, there is no evidence that either of these elements serves to target the replication complex.

Several reports have proposed that RNA structures within the PV 3' NCR function in PV replication. Jacobson et al. proposed a pseudoknot structure that involves sequences from the 3D^pol gene and the 3' NCR (28). Disruption of this proposed structure by an 8-nucleotide insertion gave rise to a mutant virus with a temperature-sensitive phenotype; however, insertions of 2 or 10 nucleotides at the same site produced viruses with wild-type growth phenotypes (57). A more extensive study designed to disrupt the putative pseudoknot structure also yielded anomalous infectivities of transfected mutated cDNAs (47). Alternatively, Pilipenko et al. proposed the existence of two stem-loops (X and Y) within the 3' NCR of poliovirus (48). The existence of these structures would preclude the formation of the pseudoknot structure. Furthermore, a proposed tertiary "kissing" interaction involving base pairing between the loop regions of stem-loops X and Y was suggested (48, 49). Transfection of transcripts containing mutations in either loop region resulted in recovered virus that contained reversion mutations or second-site compensatory mutations predicted to reestablish the "kissing" interaction. However, not all of the recovered viruses had mutations that could reestablish this interaction, and the authors suggested the possible existence of unidentified second-site compensatory mutations. While these studies suggested a role for the PV 3' NCR in genome replication, a clear mechanistic description and a precise definition of a minimal cis-acting replication element have yet to emerge.

To more clearly define the minimal boundaries of and requirements for a cis-acting replication element within the PV 3' NCR, we previously reported the deletion of the entire 3' NCR from a full-length PV cDNA construct (pT7PV3'NCR) (63). Surprisingly, transfections of transcripts harboring this complete PV 3' NCR deletion mutation (3' NCR PV1) demonstrated that, while the deletion mutation was deleterious to RNA replication, the lesion was not lethal. When deletion mutation transcripts were transfected into HeLa cells, there was a long delay before the detection of cytopathic effects (CPE) and RNA accumulation. We showed that the replication delay was not due to a defect in the accumulation of viral translation products. In contrast, virus recovered from these transfections had only a moderate RNA replication defect. The recovered viruses maintained the complete 3' NCR deletion mutation and were able to accumulate to levels 1 log₁₀ lower than wild type. Further analysis of the recovered virus suggested that there was a defect in the initiation of positive-strand RNA synthesis (8). The long delay before the abrupt appearance of newly synthesized viral RNA after transfection with pT7PV3'NCR-derived RNA, coupled with the almost-wild-type phenotype of third-passage 3' NCR PV1, suggested that a severe RNA replication defect was overcome by the accumulation of a compensatory mutation(s) generated during initial rounds of viral RNA replication.

In an attempt to identify compensatory mutations responsible for the replication phenotype of 3' NCR PV, we sequenced the entire genome of a plaque-purified isolate (4-1 M). Furthermore, to understand how identified mutations affect PV genome replication in the absence of a 3' NCR, we reconstructed the pT7PV3'NCR full-length cDNA by reverse transcription-PCR (RT-PCR) amplification of subgenomic segments of the 3' NCR PV1 genome. Here we show that a second-site compensatory mutation is not required to achieve nearly wild-type RNA replication of the deletion mutation RNA. We also show that there are no significant differences in the kinetics of translation or in the stability of the deletion mutation transcripts compared to transcripts corresponding to wild-type poliovirus genomes. In addition, we found that removing the covalently linked viral protein VPg does not affect the infectivity of deletion mutant viral RNA. However, establishing an authentic viral polyadenylated terminus increases the specific infectivity of deletion mutation transcripts, suggesting that the PV 3' NCR may be involved in site selection for initiation of negative-strand RNA synthesis.

	MATERIALS AND METHODS

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Virus stocks and plaque assay. 3' NCR PV1 mutant virus stocks were plaque isolated and passaged in HeLa (R19) monolayers as described previously (11). HeLa cell monolayers were infected with serial dilutions of virus and overlaid with semisolid minimal essential medium (MEM) containing 0.45% agarose. Well-isolated plaques were harvested. Virus was twice plaque purified and passaged three times in HeLa (R19) monolayers at 37°C to amplify the virus stocks. Plaque assays were performed as described previously (11).

One-step growth cycle analysis. One-step growth analysis was performed on HeLa (R19) monolayers in 60-mm plates at 37°C as described previously (64). HeLa cell monolayers were infected at a multiplicity of infection (MOI) of 15 for 30 min at room temperature in 60-mm plates and washed with phosphate-buffered saline, followed by the addition of 3 ml MEM plus 8% newborn calf serum with 1% nonessential amino acids. Infected-cell monolayers were harvested and virus was released from the cells by five freeze/thaw cycles, and the titer of the clarified supernatant was determined by plaque assays.

Total cellular RNA extraction. Total cytoplasmic RNA for viral genome sequencing and for use in cDNA synthesis was harvested by the Nonidet P-40, sodium dodecyl sulfate (SDS) lysis method, modified after Campos and Villarreal (10). HeLa cell monolayers were infected at an MOI of 15. At 5 to 6 h postinfection, cells were harvested and collected by centrifugation. Cells were lysed by adding Nonidet P-40-TSM buffer (0.15 M NaCl, 5 mM MgCl₂, 10 mM Tris-HCl [pH 7.6], 2% [vol/vol] Nonidet P-40). The lysate was clarified by centrifugation, and the cytoplasmic fraction was equilibrated with an equal volume of RNA extraction buffer (8 M urea, 2% SDS, 20 mM EDTA, 0.3 M NaCl, 50 mM Tris, pH 8.0). Total cytoplasmic RNA was phenol-chloroform extracted, ethanol (EtOH) precipitated, and resuspended in diethyl pyrocarbonate (DEPC)-treated H₂O.

Plasmids. A T7 bacteriophage promoter-containing plasmid encoding a genome length PV1 cDNA (pT7-PV1) (23) and a PV1 genome harboring a complete 3' NCR deletion (pT7PV3'NCR) (63) have been described previously. Synthesis of cDNA was performed as described previously (15). Plasmids containing suballelic reconstructions pT73SAR1, -2, -3, -4, and -5 were generated by RT-PCR amplification of 3' NCR PV1 (4-1 M) viral RNA genomic segments from extracted total cytoplasmic RNA using primer sets (PV genomic position is indicated in brackets) T2(+) [12 to 41]/PV2365(–) [2365 to 2384], DBPV2184(+) [2184 to 2203]/JT2C4169(–) [4169 to 4188], DBPV2992(+) [2992 to 3011]/L453(–) [5629 to 5647], PV2B(+) [3995 to 4015]/PV3D3(–) [6233 to 6252], and L449(+) [6012 to 6026]/S7181(–) [7181 to 7197], respectively. The cDNAs were cloned into the pT7PV3'NCR construct using the restriction endonuclease sites indicated in Fig. 2. Plasmid pT73SAR6 was generated by combining the NheI-to-BstEII DNA fragment of pT73SAR2, the BstEII-to-BglII DNA fragment of pT73SAR3, and the BglII-to-AccI DNA fragment of pT73SAR4 with the vector containing the AccI-to-NheI DNA fragment of pT73SAR1.

View larger version (21K): [in this window] [in a new window]   FIG. 2. Schematic map of suballelic reconstructions. The figure shows how the full-length deletion mutation cDNA, pT7PV3'NCR, was reconstructed with cDNA fragments of the third-passage 3' NCR PV1 (4-1 M) RNA. Suballelic portions of the genome were reverse transcribed, PCR amplified, and cloned into appropriate restriction sites of pT7PV3'NCR. The segments are displayed as the shaded areas, and the restriction endonucleases (and restriction site locations) used in the cloning of these suballelic reconstructions are labeled. The arrows within the shaded genomic segments indicate the location and nucleotide changes of 3' NCR PV1 (4-1 M) RNA from the parental clone. Each plasmid was linearized using restriction endonuclease EcoRI and was under the transcriptional control of a T7 bacteriophage promoter element. A genomic map of PV is displayed at the top of the panel for reference.

Genomic sequence. cDNAs generated for the construction of pT73SAR1, -2, -3, -4, and -5 were generated in duplicate to account for possible errors introduced by the DNA polymerases in the RT-PCRs. These same cDNAs were used for sequencing the 3' NCR PV1 (4-1 M) genome. The 5' end (nucleotides 1 to 100) of the 3' NCR PV1 (4-1 M) RNA genome was sequenced directly as described previously (11). The 3'-terminal sequences of the viral genome were determined via asymmetric RT-PCR and were reported previously (63). Sequences between 7100 and 7300 were sequenced from an RT-PCR-generated cDNA using the primer set PV3C(+) [5480 to 5501]/PV7350(–) [7350 –7369].

RNA transfection and specific-infectivity analysis. HeLa cell transfections were carried out with either in vitro-derived transcripts or purified virion RNA as described previously (11). Viral RNA was prepared by extraction of sucrose gradient-purified poliovirus as previously described (14, 26). HeLa cell monolayers in 60-mm plates were transfected with 200 µl of a mixture consisting of RNA (at various concentrations), 1 mg/ml DEAE-dextran, and TS buffer (137 mM NaCl, 4.4 mM KCl, 0.7 mM Na₂HPO₄, 25 mM Tris, 0.5 mM MgCl₂, 0.68 mM CaCl₂, adjusted to pH 7.45). Transfection mixtures were added to each monolayer for 30 to 40 min at room temperature. The mixtures were removed, and the monolayers were washed once with MEM plus 8% newborn calf serum with 1% nonessential amino acids. Transfected cells were then overlaid with either MEM plus 8% newborn calf serum with 1% nonessential amino acids or with semisolid 0.45% agarose media to determine specific infectivities. The transfected cells were incubated at 37°C for 2 to 4 days. Monolayers were fixed with 10% trichloroacetic acid and stained with crystal violet for plaque analysis when appropriate.

Extended poly(A) tracts were synthesized in reaction mixtures containing in vitro-derived RNAs, poly(A) polymerase reaction buffer (50 mM KCl, 0.7 mM MnCl₂, 0.2 mM EDTA, 100 µg/ml acetylated bovine serum albumin, 10% glycerol, 20 mM Tris-HCl, pH 7.0), 0.5 µM ATP, and recombinant yeast poly(A) polymerase (600 U; USB). Reaction mixtures were incubated for 20 min at 37°C, and reactions were terminated by the addition of 10 mM EDTA and incubation on ice. Quantity and integrity of RNAs were determined by 1% agarose gel separation, ethidium bromide staining, and comparison to virion RNAs of known concentration.

In vitro RNA stability. In vitro-derived ³²P-labeled transcripts were generated as described previously (53). Stability of radiolabeled transcripts was determined in a 30-µl mixture of 67% HeLa S-10 translation-replication extract (see below), radiolabeled RNAs (1.5 x 10⁴ cpm/reaction), and DEPC-H₂O (to 30 µl) in the presence or absence of 0.2 µg of cycloheximide. Reaction mixtures were incubated at 37°C, and 5-µl portions were removed at specific times. Reactions were stopped by the addition of 250 µl of a buffered SDS solution (0.5% SDS, 1 mM EDTA, 100 mM NaCl, 10 mM Tris-HCl, pH 7.5). RNA from these reactions was phenol-chloroform extracted twice, precipitated with EtOH, and pelleted at 15,000 x g for 20 min. RNA pellets were washed twice with 70% EtOH, dried, and resuspended in 40 µl of DEPC-treated H₂O. The RNAs from each reaction were separated by electrophoresis on a 1.1% agarose gel, stained with ethidium bromide, and visualized by UV illumination. The gels were dried, and the radiolabeled RNAs were detected and quantified by phosphorimager analysis (Molecular Dynamics, Sunnyvale, California).

In vitro translation. Extracts were prepared as described by Barton et al. (5) with the following minor differences (64): (i) HeLa cells were resuspended in a volume equal to that of the cell pellet using hypotonic buffer, and (ii) the initiation factor preparation used to supplement the translation reactions contained glycerol to a final concentration of 10%. In vitro translation reaction mixtures were incubated with in vitro-transcribed RNA from pT7-PV1 or pT7PV3'NCR or with purified virion PV1 RNA in the presence of 15 µCi [³⁵S]methionine and 2 mM guanidine-HCl.

Computer-predicted RNA secondary structures. Secondary structures for 3'-terminal sequences starting at position 7287 of the PV1 genome were determined using Mfold, version 3.1 (34, 75), under default settings (http://www.bioinfo.rpi.edu/applications/mfold/old/rna/). Two minimum-free-energy structures were generated for each sequence, and the structures that maintained stem-loop Y are shown in Fig. 7.

View larger version (26K): [in this window] [in a new window]   FIG. 7. Computer-modeled secondary structures of PV 3' RNA sequences with and without a 3' NCR. RNA sequences corresponding to nucleotide positions 7287 through 7441 of wild-type PV1 or nucleotide positions 7287 through 7373 of 3' NCR PV1 include 24 A residues of the 3' poly(A) tract. Minimum-free-energy values are indicated below each structure. The first stop codon is boxed in each structure, and proposed stem-loop structures X and Y of the 3' NCR are indicated on the wild-type structure.

	RESULTS

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To further characterize the growth kinetics and maximum accumulation levels of 3' NCR PV1 (4-1 M), we performed a synchronized single-cycle growth analysis by infecting HeLa cell monolayers at a high MOI with either wild-type virus or deletion-mutant virus. We harvested the cells at specific times after infection, measured the accumulation of virus, and expressed the viral titer as PFU/cell (Fig. 1). The single-cycle growth curve in Fig. 1 shows that the mutant virus accumulated at a slightly slower rate than wild-type virus. In addition, maximum mutant virus accumulation was less than that of wild type by 1 log₁₀ unit. These data could account for the small-plaque phenotype we observed on HeLa cell monolayers (8). Our data are consistent with the slightly delayed kinetics of deletion-mutant RNA accumulation following infection that we had observed previously (63). In contrast, virus replication kinetics following transfection with deletion mutation transcripts display a very significant (30- to 50-h) delay in the accumulation of virus compared to wild-type PV1 transcripts. Here we report that, following viral infection, an 1-h delay in deletion mutant virus replication kinetics was observed compared to wild-type PV1, representing a significant increase in the kinetics of viral replication and a nearly wild-type phenotype of deletion mutant virus. Because we had shown that the high-titer stock of 3' NCR PV1 maintained the complete 3' NCR deletion, these data suggested that the virus may have undergone nucleotide changes in the genome outside of the 3' NCR that resulted in an increased replicative capacity.

View larger version (13K): [in this window] [in a new window]   FIG. 1. Single-cycle growth analysis of PV1 and 3' NCR PV1. HeLa cell monolayers were infected with either wild-type PV1 (•) or 3' NCR PV1 (4-1 M) () at an MOI of 15 and incubated at 37°C, and cells were harvested at 1.5, 3, 4.5, 6, and 7.5 h postinfection. The virus titer was determined by plaque assays.

Complete genomic nucleotide sequence of 3' NCR PV1 (4-1 M).

Suballelic reconstruction of the deletion mutation cDNA. To determine if a particular mutation, or the pair of mutations, could confer greater infectivity upon deletion mutation transcripts, pT7PV3'NCR was reconstructed with suballelic segments from the 3' NCR PV1 (4-1 M) virus genome (Fig. 2). Suballelic cDNAs were generated by RT-PCR amplification of five separate segments of the third-passage 3' NCR PV1 (4-1 M) genome. The cohort of these suballelic segments represents the entire genome except for the very 5' and 3' termini. The mutations identified by complete genomic nucleotide sequencing (A5081G and U6026C) were individually contained within two separate suballelic reconstructions, pT73SAR3 and pT73SAR4, respectively. Compared to the original 3' NCR deletion construct, transcripts that contained a segment of the genome possessing a compensatory mutation might be expected to have faster growth kinetics, as evidenced by the production of CPE at an earlier time posttransfection than observed following transfection with the original pT7PV3'NCR-derived transcripts.

HeLa cell transfections were carried out with in vitro-derived transcripts produced by T7 RNA polymerase from each of the individual suballelic reconstructed cDNAs. None of the reconstructions displayed a rescue phenotype after transfection (defined by a reduced time to observed CPE) compared to transfection carried out with pT7PV3'NCR transcripts (data not shown). In addition, when transcripts containing both mutations A5081G and U6026C (pT73SAR6; Fig. 2) were used in this transfection analysis, no rescue phenotype was observed (data not shown).

Specific-infectivity analysis of virion and in vitro-derived RNAs. To provide a quantitative assessment of the putative rescue functions of pT73SAR6, we compared its specific infectivity to that of RNAs isolated from virions of both 3' NCR PV1 (4-1 M) and PV1. Since the 3' NCR PV RNAs were recovered from progeny virions, these RNAs should be infectious and contain all necessary compensatory elements required for nearly wild-type replication. We determined the specific infectivity (PFU/µg RNA) of wild-type pT7-PV1 transcripts, purified wild-type PV1 virion RNA, pT7PV3'NCR transcripts, pT73SAR6 transcripts, and purified 3' NCR PV1 virion RNA (Fig. 3). As expected, pT7-PV1 transcripts had approximately a 10-fold-lower specific infectivity than those of purified wild-type PV virion RNA (Fig. 3, compare bars 1 and 4) (25, 27, 66). The specific infectivity of either the pT7PV3'NCR or pT73SAR6 transcripts was greater than 4 log₁₀ units lower than that of wild-type transcripts. In contrast, the specific infectivity of purified deletion-mutant virion RNA was greater than 10⁴ PFU/µg RNA. The difference in the specific infectivities of virion RNA from the wild-type and deletion-mutant viruses is consistent with the single-cycle growth data obtained for these virus isolates (Fig. 1). These data demonstrate that, although the pT73SAR6 reconstruction contains a majority of the 3' NCR PV1 (4-1 M) genome sequence, including mutations A5081G and U6026C, a rescue phenotype was not detected.

View larger version (39K): [in this window] [in a new window]   FIG. 3. Specific-infectivity analysis of wild-type and 3' NCR-deleted RNAs in HeLa cell monolayers. Serial dilutions of RNA were transfected into HeLa (R19) monolayers via DEAE-dextran, and specific infectivities of RNAs were determined by plaque assay. RNAs were derived from in vitro transcription reactions (bars 1 to 3) or from purified RNA from sucrose gradient-isolated virions (bars 4 and 5). Specific infectivities represent the averages of multiple experiments performed in duplicate. Virion RNA concentration was determined by spectrophotometer readings of optical density at 260 nm, and in vitro-derived transcript RNA was quantitated by ethidium bromide staining and comparison against a poliovirus RNA standard in a 1% agarose gel.

Nonviral sequences at the termini of 3' NCR transcripts inhibit replication.

At the 3' end of the PV genome is a genetically encoded poly(A) tract that is necessary for viral RNA infectivity (61, 72, 73). In vitro-derived transcripts contain a poly(A) tract but are flanked at the 3' end by 4 nucleotides (pT7Rz3'MluI) or 7 nucleotides (pT7PV3'NCR and pT73SAR6) of nonviral vector sequences. These sequences arise as a consequence of linearizing the full-length cDNA constructs by restriction enzyme digestion in preparation for in vitro transcription reactions. We reasoned that, while the 3' nonviral sequences may pose little challenge to genomic replication in the presence of a 3' NCR, the nonviral sequences may inhibit replication of genomic RNAs that have a complete 3' NCR deletion. To address this possibility, we used yeast poly(A) polymerase to add poly(A) tracts of >200 residues to the ends of our in vitro-derived deletion mutation transcripts, thereby generating authentic 3' termini. The addition of 3' poly(A) tracts to wild-type transcripts had essentially no effect on wild-type RNA infectivity (Fig. 4A, compare bars 1 and 4). In contrast, when poly(A) polymerase was used to add a poly(A) tract to the 3' ends of in vitro-derived deletion mutation transcripts, the infectivity increased by at least 2 orders of magnitude (100- to 200-fold) over mock poly(A) polymerase-treated transcripts (Fig. 4A, compare bars 2 and 5 and 3 and 6, respectively). Furthermore, the addition of an authentic 3' poly(A) terminus to pT73SAR6 transcripts resulted in RNAs that had no increase in specific infectivity over that of pT7PV3'NCR transcripts also treated with poly(A) polymerase (Fig. 4A, compare bars 5 and 6). While the specific infectivity of poly(A) polymerase-treated over mock poly(A) polymerase-treated transcripts was 2 orders of magnitude higher, this difference may be reflective of the fact that mock-treated transcripts had lower specific infectivities than transcripts that were untreated. In addition, the specific infectivities of the treated RNAs were still below those of the isolated virion RNAs. To address the possibility that both the 5' and 3' termini need be authentic to generate transcripts with specific infectivities matching virion RNA, we generated a construct that encoded both a 5' hammerhead ribozyme and a 3' BcgI linearization restriction enzyme site. By using the BcgI site at the 3' end of the poly(A) tract, we were able to use the linearized cDNA genomic templates to generate transcripts with authentic 3' poly(A) termini. Transcripts containing authentic 5' and 3' termini were approximately fivefold more infectious than transcripts with an authentic 5' terminus alone (Fig. 4B). While these deletion mutation transcripts had the highest specific infectivities that we measured, they are still several orders of magnitude lower than those of the deletion mutant virion RNAs.

View larger version (30K): [in this window] [in a new window]   FIG. 4. Specific infectivity analysis of nonviral terminal sequences. In vitro-derived RNAs were generated from the indicated cDNA templates. Specific infectivities (PFU/µg RNA) were determined by plaque assay following DEAE-dextran-mediated transfection of transcripts into HeLa (R19) cells and are reported as the averages of at least two experiments. (A) The 3' termini of transcripts generated from the indicated cDNA constructs either were modified posttranscriptionally by the addition of an elongated poly(A) tract using poly(A) polymerase (bars 4 to 6) or remained unmodified in mock poly(A) polymerase reactions (bars 1 to 3). The specific infectivities reported by bars 2 and 3 (asterisks) were below the level of detection and therefore represent the maximum possible specific infectivities that could have been measured. (B) Both 5' and 3' nonviral sequences were eliminated from in vitro-derived transcripts by the use of a Klenow-treated BcgI-linearized cDNA template encoding a 5' hammerhead ribozyme (bar 2). The infectivity of these transcripts is contrasted to transcripts that have an authentic 5' terminus but contain nonviral sequences at the 3' terminus (bar 1). (C) The ethidium bromide-stained agarose gel shows a shift in the sizes of poly(A) polymerase-treated RNA transcripts (lanes 3, 5, and 7) compared to those of the mock-treated transcripts (lanes 2, 4, and 6), demonstrating that poly(A) polymerase added additional poly(A) tracts to the 3' ends of these transcripts. Purified PV1 virion RNA is shown as a marker in lane 1.

View larger version (64K): [in this window] [in a new window]   FIG. 5. In vitro translation kinetics of wild-type (wt) and 3' NCR transcript RNAs. Translation and processing were carried out in HeLa cell extracts at 30°C in the presence of [35S]methionine. Extracts were incubated with PV1 virion RNA (lane 1) or no RNA (lane 2) for 4 h. At the indicated times, 10-µl portions of the extracts incubated with pT7-PV1-derived transcripts (lanes 3 to 8) or pT7PV3'NCR-derived transcripts (lanes 9 to 14) were removed and translation was terminated by the addition of Laemmli sample buffer (31) and boiling for 3 to 5 min. These products were analyzed on an SDS-2.5% polyacrylamide gel and visualized by phosphorimager (Personal Molecular Imager FX; Bio-Rad, Hercules, California).

Stability of in vitro-derived 3' NCR transcripts.

View larger version (36K): [in this window] [in a new window]   FIG. 6. Wild-type and deletion mutation transcript stability in HeLa S10 extracts. Transcript stability was determined as described in Materials and Methods. (A) HeLa S10 extracts were incubated with radiolabeled wild-type (lanes 3 to 10) or deletion mutation (lanes 11 to 18) transcripts in the presence (lanes 3 to 7, 9, 11 to 15, and 17) or absence (lanes 8, 10, 16, and 18) of cycloheximide. PV virion RNA (lane 1) or a radiolabeled PV transcript (lane 2) was loaded as the marker. At the indicated times, portions of the extract mixture were removed and the RNA was phenol-chloroform extracted. Total RNA was separated by electrophoresis on a 1.1% agarose gel and visualized by ethidium bromide staining and UV illumination (data not shown). The gel was dried, and radiolabeled products were visualized and quantitated by phosphorimager analysis (Personal Molecular Imager FX; Bio-Rad, Hercules, California). *, lane containing a sample overloaded on the gel by 20% compared to other samples and rRNA loading controls. (B) Products correlating to full-length genomic RNA incubated in the presence of cycloheximide were normalized to input (zero time) levels and plotted on a graph.

	DISCUSSION

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Our previous studies with PV transcripts lacking a 3' NCR had raised the possibility that, during initial low-level RNA replication following transfections, compensatory mutations had accumulated in the deletion-mutant genome (63). Sequencing through the 3' NCR lesion did not identify reversion mutations, indicating that putative compensatory mutations may have arisen elsewhere in the genome. Complete nucleotide sequencing of the genomic RNA from a third-passage virus stock revealed two nucleotide changes from the parental genomic sequence. These nucleotide changes resulted in amino acid changes in both the 2C and 3D proteins. When transcripts from a pT73SAR6 expression clone, containing both of the identified mutations, were transfected into HeLa cells, there was no reduction in the time to observed CPE, nor was there an increase in RNA specific infectivity. However, there was an increase in the specific infectivities of deletion mutation transcripts when the 5' and/or the 3' termini of the 3' NCR transcripts were modified to mimic those of virion RNA. While wild-type poliovirus transcripts containing an authentic 5' end are known to have a higher specific infectivity than genomic transcripts that contain nonviral sequences at their 5' termini (25, 27, 66), the generation of wild-type transcripts with authentic 3' poly(A) termini does not significantly increase their specific infectivities. An increase in infectivity due to an authentic 3' terminus was unique to the deletion mutation RNAs and suggested that efficient initiation of deletion mutant negative-strand RNA synthesis is mediated through an authentic poly(A) 3' terminus. Although both the 3' poly(A) tract and the 3' NCR of cellular mRNAs have been shown to be involved in translation and stability modulation, the deletion mutation transcripts were shown to be nearly identical to wild-type transcripts in both genome stability and translation efficiencies. Thus, while the addition of an authentic 3' poly(A) terminus resulted in an increase in specific infectivity of deletion mutation transcripts, this increase was not due to a compensatory effect on RNA stability or translation and viral polypeptide processing. The equal specific infectivities of pT7PV3'NCR- and pT73SAR6-derived transcripts, terminating in adenosine nucleotides or not, confirmed that 3' NCR PV viral RNA does not contain compensatory mutations.

The reason for the much higher infectivity of deletion mutant virion RNA over that of the deletion mutation transcript RNA remains unclear. Based the our data showing that deletion mutant virion RNAs had specific infectivities within 1 log unit of those observed for wild-type virion RNAs (Fig. 3), we conclude that the mode of entry of the RNA into the cell (i.e., transfection versus infection) cannot account for this difference. It may be that the poly(A) tract needs to be of a precise length for optimal infectivity. However, the specific infectivities of deletion mutation RNAs with 16 (data not shown), 27, and 51 (this study) adenosine residues are essentially identical, while pT7Rz3'BcgI-derived transcripts have 46 adenosine residues but are more infectious than the original deletion mutant transcripts. Another possibility for the increased infectivity of virion RNA is that epigenetic information may be contained within the deletion mutant virion RNA. Such epigenetic information might take the form of an RNA structural element that requires a chaperone-like factor(s) to properly form (during RNA replication in the cytoplasm of infected cells) or perhaps the inclusion of modified nucleotide moieties that may be found within the infected cell. Alternatively, there could be an inhibitory RNA structure(s) or component(s) associated with generating genomic RNAs in vitro in the absence of host cell components. This putative epigenetic component would appear to be of no consequence in wild-type RNAs; however, in the absence of the RNA sequences and structures contained within the 3' NCR, such a component may take on added importance.

Previous reports have provided speculation on the severity of the replication defect of our mutant virus harboring a complete 3' NCR deletion during infection of HeLa cells (1, 46, 51, 67). Although the specific steps in RNA replication affected by the deletion are still under investigation, it is now clear that growth of this virus does not require second-site compensatory mutations (i.e., PV3'NCR is infectious in contrast to quasi-infectious). While the 3' NCR is not absolutely necessary for PV genomic RNA replication, data presented in this study showed that the 3' NCR has a functional role in RNA replication since the deletion-mutant virus does not achieve wild-type replication levels. Previous studies examining the role of picornavirus 3' NCRs in viral replication have come to similar conclusions (16, 28, 37, 38, 47-49, 55, 57). Moreover, we have recently shown that the poliovirus genomic 3' NCR has a cell-dependent role in the initiation of positive-strand RNA synthesis (8). Apart from these previous findings, this study implicates the 3' NCR in the role of nonterminal synthesis initiation of negative-strand RNA intermediates during PV RNA replication. We speculate that, when the 3' NCR is intact, negative-strand RNA synthesis can initiate at a number of sites along the poly(A) tract, possibly by maintaining the position of the VPg protein primer. However, when the 3' NCR contains a severe lesion or is completely deleted, initiation may be confined to the very 3' terminus of the poly(A) tract. Therefore, we propose that the PV genomic 3' NCR plays a role in multiple steps of RNA replication, affecting both positive-strand and negative-strand RNA synthesis. Point mutations and small deletions within the 3' NCRs of enterovirus RNAs have been reported to be lethal (37, 39). We suggest that such lesions within the 3' NCR disrupt a functional element that is recognized by factors involved in RNA replication complex formation, resulting in the misdirection of such factors to generate nonfunctional RNA replication complexes.

The deletion of the 3' NCR of poliovirus RNA may only partially disrupt a cis-acting replication element that is constructed from multiple RNA structures. When the 3' NCR is completely removed, the remaining element is sufficient to function, albeit at slightly less than wild-type levels. We examined computer-predicted structures of the 3' ends of PV and 3' NCR RNAs, including the 3'-most nucleotides of the 3D^pol coding sequence (Mfold V3.1) (34, 75). When we compared the predicted RNA secondary structures of wild-type and 3' NCR deletion mutation PV RNAs, we found that the complete deletion of the 3' NCR leads to a precise removal of predicted stem-loops X and Y but leaves a larger stem-loop structure in the 3D coding region unaffected (Fig. 7, compare wild type to 3' NCR). This predicted 3D stem-loop structure is conserved among the three serotypes of PV (data not shown). Such a structure may represent a minimal replication element that, in concert with the 3' NCR, forms a larger tertiary structure required for maximum levels of RNA replication.

It has been proposed that a cis-acting targeting element may not be necessary to assure accurate replication of the viral genome (12, 63). Novak and Kirkegaard showed that genomic RNA must be translated in order for it to be replicated (42). Furthermore, nascent nonstructural (P2 and P3) gene products are proximal to the 3' terminus of RNAs from which the proteins are translated (50). Given the tight membrane association of RNA replication functions (62), it is not hard to imagine that an important cis signal for negative-strand RNA synthesis may be the proximal translation of viral nonstructural proteins. Furthermore, positive-strand RNA synthesis may require the completion of a negative-strand intermediate as a cis signal for replication. Finally, it has been shown that genomic replication and packaging are coupled (4, 43, 65), suggesting that each step in virus replication may be a signal that mediates the onset of the next step in the virus life cycle.

	ACKNOWLEDGMENTS

 
We acknowledge the DNA Core Automated DNA Sequencing Facility and its support from the UCI Cancer Center and the UCI School of Biological Sciences. D.M.B. and C.T.C. were predoctoral trainees supported by Public Health Service training grant AI 07319. This work was supported by Public Health Service grant AI 22693 from the National Institutes of Health.

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Microbiology and Molecular Genetics, School of Medicine, University of California, Irvine, CA 92697. Phone: (949) 824-7573. Fax: (949) 824-2694. E-mail: blsemler{at}uci.edu.

Present address: Department of Molecular Biology, Princeton University, Princeton, NJ 08544.

Present address: Department of Molecular and Integrative Neuroscience, The Scripps Research Institute, La Jolla, CA 92037.

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